Constraining and Modifying Peptides Using Pd‐Mediated Cysteine Allylation

Author:

Kriegesmann Julia1ORCID,Schlatzer Thomas2,Che Kateryna1,Altdorf Claudia3,Huhmann Susanne1,Kählig Hanspeter4ORCID,Kurzbach Dennis1ORCID,Breinbauer Rolf2ORCID,Becker Christian F. W.1ORCID

Affiliation:

1. Institute of Biological Chemistry Faculty of Chemistry University of Vienna 1090 Vienna Austria

2. Institute of Organic Chemistry Graz University of Technology 8010 Graz Austria

3. Syntab Therapeutics GmbH Pauwelstrasse 17 post code? Aachen Germany

4. Department of Organic Chemistry Faculty of Chemistry University of Vienna 1090 Vienna Austria

Abstract

AbstractOver the past decades, several strategies for inducing and stabilizing secondary structure formation in peptides have been developed to increase their proteolytic stability and their binding affinity to specific interaction partners. Here, we report how our recently introduced chemoselective Pd‐catalyzed cysteine allylation reaction can be extended to stapling and how the resulting alkene‐containing staples themselves can be further modified to introduce additional probes into such stabilized peptides. The latter is demonstrated by introducing a fluorophore as well as a PEG moiety into different stapled peptides using bioorthogonal thiol‐ene and Diels‐Alder reactions. Furthermore, we investigated structural implications of our allyl staples when used to replace conformationally relevant disulfide bridges. To this end, we chose a selective binder of integrin α3β1 (LXY3), which is only active in its cyclic disulfide form. We replaced the disulfide bridge by different stapling reagents in order to increase stability and binding affinity towards integrin α3β1.

Funder

Austrian Science Fund

Universität Wien

Publisher

Wiley

Subject

Organic Chemistry,Molecular Biology,Molecular Medicine,Biochemistry

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